Figure 1
Figure 1. Lymphodepletion followed by the transfer of TNs induces TEs in TDLNs and inhibits tumor progression. (A) Mice were irradiated with 500 cGy and injected intravenously with 40 × 106 spleen cells from naive mice. These mice were then inoculated subcutaneously with 1 × 105 of MCA205 tumor cells along the midline of the abdomen. The resultant skin tumors were measured in 2 perpendicular directions 2 to 3 times per week, and the tumor areas (mm2) were recorded. (B) Sublethally irradiated lymphopenic mice were reconstituted with either Thy1.2, CD4, or CD8-depleted cell populations and then inoculated subcutaneously with MCA205 tumor cells. The depletion of Thy1.2+ or CD4+ cells, but not the depletion of CD8+ cells, abrogated the antitumor effects observed after lymphodepletion and reconstitution. (C) Sublethally irradiated mice (500cGy) were injected intravenously with either 40 × 106 whole spleen cells or with 10 × 106 magnetically isolated splenic TNs. Mice were then inoculated SD with MCA205 tumor cells to stimulate the TDLNs. Twelve days later, TDLN cells were harvested and activated in vitro with the method of CD3/IL-2 for 5 days. Ten million of activated TDLN cells were then adoptively transferred into a new group of mice with 3-day established pulmonary metastases. The TDLN cells from the mice reconstituted with whole-spleen cells and splenic TNs exhibited similar therapeutic effects. (D) Congenic Ly5.1+ spleen cells were labeled with CFSE and transferred into irradiated lymphopenic mice. These mice were then inoculated SD with 3 × 106 tumor cells to stimulate the TDLNs. Twelve days later, TDLNs, NDLNs, and spleens were harvested and analyzed for CFSE staining intensity within the Ly5.1+ subset.

Lymphodepletion followed by the transfer of TNs induces TEs in TDLNs and inhibits tumor progression. (A) Mice were irradiated with 500 cGy and injected intravenously with 40 × 106 spleen cells from naive mice. These mice were then inoculated subcutaneously with 1 × 105 of MCA205 tumor cells along the midline of the abdomen. The resultant skin tumors were measured in 2 perpendicular directions 2 to 3 times per week, and the tumor areas (mm2) were recorded. (B) Sublethally irradiated lymphopenic mice were reconstituted with either Thy1.2, CD4, or CD8-depleted cell populations and then inoculated subcutaneously with MCA205 tumor cells. The depletion of Thy1.2+ or CD4+ cells, but not the depletion of CD8+ cells, abrogated the antitumor effects observed after lymphodepletion and reconstitution. (C) Sublethally irradiated mice (500cGy) were injected intravenously with either 40 × 106 whole spleen cells or with 10 × 106 magnetically isolated splenic TNs. Mice were then inoculated SD with MCA205 tumor cells to stimulate the TDLNs. Twelve days later, TDLN cells were harvested and activated in vitro with the method of CD3/IL-2 for 5 days. Ten million of activated TDLN cells were then adoptively transferred into a new group of mice with 3-day established pulmonary metastases. The TDLN cells from the mice reconstituted with whole-spleen cells and splenic TNs exhibited similar therapeutic effects. (D) Congenic Ly5.1+ spleen cells were labeled with CFSE and transferred into irradiated lymphopenic mice. These mice were then inoculated SD with 3 × 106 tumor cells to stimulate the TDLNs. Twelve days later, TDLNs, NDLNs, and spleens were harvested and analyzed for CFSE staining intensity within the Ly5.1+ subset.

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